Multimerization of a disordered kinetochore protein promotes accurate chromosome segregation by localizing a core dynein module

Author:

McGory Jessica M.12ORCID,Verma Vikash1ORCID,Barcelos Dylan M.1ORCID,Maresca Thomas J.12ORCID

Affiliation:

1. University of Massachusetts 1 Biology Department, , Amherst, MA, USA

2. University of Massachusetts 2 Molecular and Cellular Biology Graduate Program, , Amherst, MA, USA

Abstract

Kinetochores connect chromosomes and spindle microtubules to maintain genomic integrity through cell division. Crosstalk between the minus-end directed motor dynein and kinetochore–microtubule attachment factors promotes accurate chromosome segregation by a poorly understood pathway. Here, we identify a linkage between the intrinsically disordered protein Spc105 (KNL1 orthologue) and dynein using an optogenetic oligomerization assay. Core pools of the checkpoint protein BubR1 and the adaptor complex RZZ contribute to the linkage. Furthermore, a minimal segment of Spc105 with a propensity to multimerize and which contains protein binding motifs is sufficient to link Spc105 to RZZ/dynein. Deletion of the minimal region from Spc105 compromises the recruitment of its binding partners to kinetochores and elevates chromosome missegregation due to merotelic attachments. Restoration of normal chromosome segregation and localization of BubR1 and RZZ requires both protein binding motifs and oligomerization of Spc105. Together, our results reveal that higher-order multimerization of Spc105 contributes to localizing a core pool of RZZ that promotes accurate chromosome segregation.

Funder

National Institutes of Health

UMass Biotechnology Training Program

Publisher

Rockefeller University Press

Subject

Cell Biology

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